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β-COP主要定位于外分泌胰腺的顺式高尔基体一侧。

Beta-COP localizes mainly to the cis-Golgi side in exocrine pancreas.

作者信息

Oprins A, Duden R, Kreis T E, Geuze H J, Slot J W

机构信息

Department of Cell Biology, Medical School, Utrecht University, The Netherlands.

出版信息

J Cell Biol. 1993 Apr;121(1):49-59. doi: 10.1083/jcb.121.1.49.

Abstract

We examined the distribution of the non-clathrin-coated vesicle-associated coat protein beta-COP in rat exocrine pancreatic cells by immunogold cytochemistry. Labeling for beta-COP was found in the Golgi region (48%) where it was associated with vesicles and buds of approximately 50 nm, showing a characteristic approximately 10-nm-thick coat. The other half of the label was present in the cytoplasm, not associated with visible coats or membranes, with a minor fraction present on small clusters of tubules and vesicles. Clathrin-coated vesicles were typically located at the trans-side of the Golgi complex, and showed a thicker coat of approximately 18 nm. Of the total beta-COP labeling over the Golgi region, 68% occurred on the cis-side, 6% on the cisternae, 17% on the rims of the cisternae, and only 9% on the trans-side. For clathrin these figures were 16, 2, 4, and 78%, respectively. At the cis-Golgi side beta-COP was present in transitional areas (TA), on so-called peripheral elements (PE), consisting of tubules and vesicles located between the cup-shaped transitional elements (TE) of the RER and the cis-most Golgi cisternae. Label for Sec23p was also present in TA but was located closer to the TE, while beta-COP labeled PE were located near the cis-Golgi cisternae. Upon energy depletion, Golgi associated beta-COP was almost exclusively (86%) in spherical aggregates of 200-500 nm in diameter, whereas the cis-side (6%), the cisternae (1%), the rims (4%) and trans-side (3%) of the Golgi complex, were barely labeled; 50% of the total label remained in the cytoplasm. The aggregates were predominantly located at the cis-side of the Golgi stack, next to, but distinct from the Sec23p positive TA, that were devoid of beta-COP and had only a few recognizable vesicles left. Incubation with aluminum fluoride resulted in fragmentation of the Golgi complex into large clusters of beta-COP positive vesicles, while 50% of the label remained in the cytoplasm, as in control cells. After 10 min of Brefeldin A treatment 91% of beta-COP was cytoplasmic and only 7% associated with membranes of the Golgi complex. The total label for beta-COP over exocrine cells remained unchanged during the incubation with either of the drugs, indicating that the drugs induce reallocation of beta-COP. Our data suggest that beta-COP plays a role in membrane transport at the cis-side of the Golgi complex.

摘要

我们通过免疫金细胞化学方法研究了大鼠外分泌胰腺细胞中非网格蛋白包被囊泡相关的包被蛋白β-COP的分布情况。在高尔基体区域发现了β-COP的标记(占48%),它与直径约50nm的囊泡和芽相关联,呈现出约10nm厚的特征性包被。另一半标记存在于细胞质中,与可见的包被或膜不相关,一小部分存在于小管和囊泡的小簇上。网格蛋白包被囊泡通常位于高尔基体复合体的反式面,呈现出约18nm厚的更厚包被。在高尔基体区域的总β-COP标记中,68%出现在顺式面,6%出现在潴泡,17%出现在潴泡边缘,而只有9%出现在反式面。对于网格蛋白,这些数字分别为16%、2%、4%和78%。在顺式高尔基体侧,β-COP存在于过渡区域(TA),在所谓的周边元件(PE)上,这些元件由位于糙面内质网杯状过渡元件(TE)和最顺式高尔基体潴泡之间的小管和囊泡组成。Sec23p的标记也存在于TA中,但位置更靠近TE,而标记有β-COP的PE位于靠近顺式高尔基体潴泡处。能量耗尽后,与高尔基体相关的β-COP几乎全部(86%)存在于直径200 - 500nm的球形聚集体中,而高尔基体复合体的顺式面(6%)、潴泡(1%)、边缘(4%)和反式面(3%)几乎没有标记;总标记的50%仍留在细胞质中。聚集体主要位于高尔基体堆栈的顺式侧,紧邻但不同于Sec23p阳性的TA,TA中没有β-COP,只剩下少数可识别的囊泡。用氟化铝孵育导致高尔基体复合体破碎成β-COP阳性囊泡的大簇,而50%的标记仍留在细胞质中,与对照细胞一样。用布雷菲德菌素A处理10分钟后,91%的β-COP位于细胞质中,只有7%与高尔基体复合体的膜相关。在与任何一种药物孵育期间,外分泌细胞中β-COP的总标记保持不变,表明药物诱导了β-COP的重新分配。我们的数据表明,β-COP在高尔基体复合体顺式侧的膜运输中起作用。

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